An improved ELISA for the determination of tobacco mosaic virus with linear sweep voltammetry detection based on a new system of PAP-H2O2-HRP

An improved ELISA for the determination of tobacco mosaic virus (TMV) with linear sweep voltammetry based on a new system of p-aminophenol (PAP)- H₂O₂- horseradish peroxidase (HRP) has been developed. The enzymatic product 3-[(4-hydroxyphenyl)amino]-4-(2-amino-5-hydroxyphenyl)-6-[(4-hydroxyphenyl)imino]-2,4-cyclohexadiene-1-one, produced from HRP catalyzing the oxidation of PAP with H₂O₂, yields a sensitive linear sweep voltammetric response at a potential of –0.45 V (vs. SCE) in Britton-Robinson (BR) buffer solution. By using this voltammetric peak, HRP can be measured with a detection limit of 0.4 mU/L and a linear range of 1.0 ∼ 1.0 × 10² mU/ L. The detection limit for the clarified TMV is 4.0 ng/mL and the highest dilution ratio detected for the infected leaf sap is 1 : 3.9 × 10⁶. The processes of the enzyme-catalyzed reaction and the electro-reduction of the product of the enzyme-catalyzed reaction have been investigated. Received: 17 November 1998 / Revised: 17 March 1999 / Accepted: 20 March 1999     

An improved ELISA for the determination of southern bean mosaic virus with linear sweep voltammetry detection based on new system of PAP-H_2O_2-HRP

An improved enzyme-linked immunosorbent assay (ELISA) for the determination of southern bean mosaic virus (SBMV) with linear sweep voltammetry based on a new system of p-aminophenol (PAP)-H2O2-horseradish peroxidase (HRP) has firstly been developed. The enzymatic product 3-[(4-hydrox-yphenyl) amino]-4-(2-amino-5-hydroxyphenyl)-6-[ (4-hydrox-yphenyl)imino]-2,4-cyclohexadiene-l-one, produced from the oxidation of PAP with H2O2 catalyzed by HRP, yielded a sensitive linear sweep voltammetric response at - 0.45 V ( vs. SCE) in Britton-Robinson (BR) buffer solution. Based on the voltammetric peak, HRP can be measured with a detection limit of 0.4 mU/L and a linear range of 1.0-1.0 × 102 mU/ L. The detection limit for the SBMV is 8.0 ng/mL and the highest dilution ratio for the detection of infected leaf sap is 1: 1.5×105.     

Enzyme-catalyzed reaction of voltammetric enzyme-linked immunoassay system based on OAP as substrate

The o-aminophenol (OAP)-H_2O_2-horseradish peroxidase (HRP) voltammetric enzyme-linked immunoassay new system has extremely high sensitivity. HRP can be measured with a detection limit of 6.0×10~-(10) g/L and a linear range of 1.0×10~(-9)—4.0×10~(-6) g/L. The pure product of H_2O_2 oxidizing OAP catalyzed by HRP was prepared with chemical method. The enzyme-catalyzed reaction has been investigated with electroanalytical chemistry, UV/Vis spectrum, IR spectrum, ~(13)C NMR, ~1H NMR, mass spectrum, elemental analysis, etc. Under the selected enzyme-catalyzed reaction conditions, the oxidation product of OAP with H_2_O2 catalyzed by HRP is 2-aminophe-noxazine-3-one. The processes of the enzyme-catalyzed reaction and the electroreduction of the product of the enzymecatalyzed reaction have been described.     

Detection of TMV with ODA-H(2)O(2)-HRP voltammetric enzyme-linked immunoassay system

o-Dianisidine (ODA)-H₂O₂-horseradish peroxidase (HRP) voltammetric enzyme-linked immunoassay system has firstly been used for the detection of tobacco mosaic virus (TMV). HRP catalyzes strongly the oxidation reaction of ODA by H₂O₂, the product of which produces a sensitive second order derivative linear sweep voltammetric peak at potential of −0.56 V (versus SCE) in Britton–Robinson (BR) buffer. HRP activity has been measured with this voltammetric peak and TMV detected through immunoreaction. The detection limit for HRP is 9.25×10^-7 mU l⁻¹ and the linear range is 2.5×10⁻⁶–5.0×10⁻⁴ mU l⁻¹. The detection limit for the clarified TMV is 0.25 ng ml⁻¹ and the highest dilution ratio detected for the infected leaf sap is 1:8×10⁵. The sensitivity for TMV detection with this method is higher than that with the enzyme-linked immunosorbent spectrophotometric assay (ELISA) using ODA-H₂O₂-HRP system. The processes of the enzyme-catalyzed reaction and the electro-reduction of the product of the enzyme-catalyzed reaction have been described.     

Electrochemical studies of 1,5-dihydroxynaphthalene as substrate for voltammetric enzyme immunoassay

Immunoassay is one of the biochemical analytical techniques using the specific antigen antibody com-plexation for analytical purposes. It has extensive ap-plication in clinical diagnostics, prevention and cure of diseases, and virus diagnostics. The presentation and progress of immunoassay methodology are one of the greatest achievements of bioanalytical chemistry. It is estimated that several-hundred millions of immuno-analytical determinations are carried out every year all over the world. E…     

Comparison of Electrochemical and Spectro-Photometric Detection in Hrp-Based Elisa for Tobacco Mosaic Virus

ABSTRACT

An electrochemical method was compared with a spectrophotometric method using a horseradish peroxidase (HRP)-based indirect enzyme-linked immunosorbent assay (ELISA) with direct antigen coating (DAC) technique for the determination of tobacco mosaic virus (TMV). In substrates for a spectrophotometric HRP-based ELISA method, was selected as the substrate for the electrochemical method as well as the spectrophotometric method. 2, 3-Diaminophenazine is the product of the oxidation of OPD with H₂O₂ catalyzed by HRP in the selected conditions. It is electroactive and has a sensitive voltammetric response at -0.93 V (vs. Ag/AgCl) in alkaline solution. The detection limit of free HRP, by second-order derivative linear-sweep voltammetry, is 1.1 mU/L. This method can be further used to detect TMV antigen. The peak current is linear with TMV concentration in the range of 0.25-5.0 ng/mL. The detection limit for TMV is 0.25 ng/mL and the highest dilution ratio detected for the infected leaf sap is 1:102400. Compared with the classical OPD ELISA spectrophotometric method, the detection limits of the electrochemical method for the clarified TMV and the infected leaf sap detection are about ten and four times lower, respectively.     

MAP-H~2O~2-HPR伏安酶联免疫分析新体系和光谱及电化学研究

提出了间氨基酸(MAP)-H~2O~2-辣根过氧化物酶(HRP)伏安酶联免疫分析新体系.本方法以线性扫描二阶导数伏安法检测HRP催化H~2O~2氧化MAP的产物,用于游离HRP和各种HRP标记物的测定,灵敏度均高于经典的ELISA显色光度法.测定游离HRP的线性范围为1.0x10^-^8-1.0x10-6/L,检测限达3.8x10^-^9g/L.制备出了HRP催化H~2O~2氧化MAP的产物纯品并应用电化学分析,高效液相色谱,元素分析,紫外-可见光谱,红外光谱,^1H核磁共振谱,^1^3C核磁共振谱及质谱等技术对体系酶促反应进行了深入的研究.在选择的酶促反应条件下,生成的产物为2-氨基-5-[(3-差苯基)]-2,5-环己烯基-1,4-二酮.提出了酶催化反应机理及其产物的电极还原过程。     

PAP-H2O2-HRP酶促反应产物光谱及电化学研究

前文［１］首次提出了以对氨基酚（ＰＡＰ）为底物的ＰＡＰ－Ｈ２Ｏ２－辣根过氧化物酶（ＨＲＰ）伏安酶联免疫分析新体系,并成功地应用于烟草花叶等植物病毒的血清学检测．在此之前,我们也曾报道过一些伏安酶联免疫分析新体系［２,３］．迄今,还没有人对 ＨＲＰ催化 Ｈ２Ｏ２氧化 ＰＡＰ的酶促反应进行过探讨．Ｐｒａｔｉ等［４］报道了在铜催化作用下,Ｏ２氧化对氨基酚生成３－［（４－个羟苯基）氨基」－４－（２－氨基－５－羟苯基）－６－［（４－羟苯基）亚胺基］－２,４－环己二烯基－１－酮．本文的实验结果与此文献不符． 为…     

Detection of ferritin in human serum with a MAP-H(2)O(2)-HRP voltammetric enzyme-linked immunoassay system

A voltammetric enzyme-linked immunoassay based on new system of m-aminophenol (MAP)-H(2)O(2)-horseradish peroxidase (HRP) has firstly been developed and used for the detection of HRP, labelled HRP and ferritin in human serum. HRP or labelled HRP catalyzes the oxidation reaction of MAP with H(2)O(2), the product of which produces a sensitive voltammetric peak at potential of -0.46 V (vs. SCE) in Britton-Robinson (BR) buffer solution. By using this voltammetric peak, HRP can be measured with a detection limit of 9.5x10(-1) mU/l and a linear range of 2.5-2.5x10(2) mU/l. The detection limit to ferritin is 0.25 ng/ml and the linear range 0.25-320 ng/ml. The processes of the electro-reduction of the product of the enzyme-catalyzed reaction have been investigated in detail.     

Enzyme-catalyzed reaction of OPD-H202-HRP voltammetric enzyme-linked immunoassay system

Enzyme-catalyzed reaction of o-phenylenediamine (OPD)-H_z0₂-horseradish peroxidase (HRP) voltammetric enzyme-linked immunoassay system has been studied in detail with electrochemical analysis, high performance liquid chromatography (HPLC), ultraviolet/visible (UV/Vis) spectroscopy, infrared (IR) spectroscopy and nuclear magnetic resonance (NMR) spectroscopy. The pure product of H₂0₂ oxidizing OPD catalyzed by HRP was prepared with chemical method. The experimental results of voltammetry and HPLC indicate that only one product of enzyme-catalyzed reaction has been obtained under the selected enzyme-catalyzed reaction conditions. Identifications by UV/ Vis spectrum, IR spectrum and¹³C NMR spectrum show that the product is 2,3-diaminophenazine. The processes of the enzyme-catalyzed reaction and the electroreduction of the product of the enzyme-catalyzed reaction are described. Project supported by the National Natural Science Foundation of China     

Electrochemical Enzyme‐Linked Immunoassay for the Determination of Estriol Using Methyl Red as Substrate

Abstract

A new electrochemical substrate for horseradish peroxidase, methyl red, is reported. In this reaction system, horseradish peroxidase can catalyze the redox reaction of methyl red and H₂O₂. Methyl red exhibits a sensitive voltammetric peak at?0.51 V vs. Ag/AgCl reference electrode, the decrease of the peak current of methyl red is in proportion to the concentration of horseradish peroxidase (HRP). The linear range for determination of horseradish peroxidase is 5.0×10^?8～5.0×10^?7 g mL^?1 and the detection limit is 1.8×10^?8 g mL^?1. The relative standard deviation is 3.3% when 2.0×10^?7 g mL^?1 HRP was sequentially determined 11 times. A voltammetric enzyme‐linked immunoassay method for the determination of estriol was developed, based on this electrochemical system. The linear range for determination of estriol is 1.0～1000.0 ng mL^?1, and the detection limit is 0.33 ng mL^?1. The relative standard deviation for 11 parallel determinations with 200 ng mL^?1 estriol is 4.8%. Some pregnancy serum samples were analyzed with satisfactory results.     

Characterization of a Layered Methylene Blue/Vanadium Oxide Nanocomposite and its Application in a Reagentless H2O2 Biosensor

Layered nanocomposite of methylene blue (MB)-intercalated vanadium oxide was obtained through a simple hydrothermal synthesis method using MB, V₂O₅, and NaI as starting materials. The intercalation reaction was proven to be successful using X-ray diffraction pattern. The MB-V₂O₅ nanocomposite was characterized using a scanning electron micrograph, infrared spectra, thermogravimetric analysis, UV spectra, and electrochemical measurements. The intercalated MB cations showed a fine diffusion-controlled electrochemical redox process and facilitated the immobilized horseradish peroxidase’s (HRP) good catalytic reduction upon H₂O₂. The as-prepared MB-V₂O₅/HRP biosensor showed a linear response to H₂O₂ over a range from 2.0?×?10^?6 to 9.5?×?10^?5 M with a detection limit of 9.7?×?10^?7 M (S/N ratio?=?3).     

Kinetics of phenol oxidation by peroxidase

Studies of the kinetic behavior of horseradish peroxidase (HRP) at pH 8 and at room temperature indicate that the reaction of phenol with H₂O₂ catalyzed by HRP exhibits normal Michaelis-Menten saturation kinetics. An irreversible reaction mechanism for the steady-state kinetics of HRP, which is consistent with the experimental data, is considered. The second-order rate constants for the reactions of HRP with H₂O₂ and compound II with phenol are 4.14 × 10⁵ M^-1s^-1 and 5.54 × 10⁴M^-1s^-1, respectively.     

Direct Electrochemistry of Horseradish Peroxidase Embedded in Nano－Fe304 Matrix on Paraffin Impregnated Graphite Electrode and Its Electrochemical Catalysis for H2O2

Fe3O4 particles coated with acrylic copolymer (ACP) of about 5--8 nm in diameter were synthesized and used for immobilization of horseradish peroxidase (HRP). Direct electrochemistry of HRP embedded in the nanosized Fe304 solid matrix modified paraffin impregnated graphite electrode (PIGE) was achieved,which is related to the heine Fe(Ⅲ)/Fe(Ⅱ) conversion of HRP. Cyclic voltammetry gave a pair of reproducible and welldefined redox peaks at about Ea of -0.295 V vs. SCE. The standard rate constant k, was determined as 2.7 s^-1. It demonstrated that the nano-Fe3O4 solid matrix offers a friendly platform to assemble the HRP protein molecules and enhance the electron transfer rate between the HRP and the electrode. UV-Vis absorption spectra and WrIR spectra studies revealed that the embedded HRP retained its native-like structure. The HRP/Fe3O4/PIGE showed a strong catalytic activity toward H2O2. The voltammetric response was a linear function of H2O2 concentration in the range of 10-140μmol/L with detection limit of 7.3 μmol/L (s/n = 3 ). The apparent Michaelis-Menten constant is calculated to be 0.42 mmol/L.     

联苯胺-H_2O_2-HRP伏安酶联免疫分析体系测定植物病毒TMV和TRSV

提出了联苯胺－Ｈ２Ｏ２－辣根过氧化物酶（ＨＲＰ）伏安酶联免疫分析体系测定植物病毒烟草花叶病毒（ＴＭＶ）和烟草环斑病毒（ＴＲＳＶ）的新方法。ＨＲＰ标记的羊抗兔酶标记抗体ＩｇＧ－ＨＲＰ可以催化Ｈ２Ｏ２氧化联苯胺的反应,其氧化产物在Ｂｒｉｔｏｎ－Ｒｏｂｉｎｓｏｎ（ＢＲ）缓冲溶液中在－０．６２Ｖ（ＳＣＥ）左右产生灵敏的线性扫描二阶导数伏安峰,可以测定ＩｇＧ－ＨＲＰ。根据ＩｇＧ－ＨＲＰ与植物病毒及其抗血清的免疫反应,可以间接测定植物病毒。本法测定ＴＭＶ的检出限为０．２５ｎｇ／ｍＬ,线性范围为０．２５～５０００ｎｇ／ｍＬ;测定ＴＲＳＶ的检出限为１．５ｎｇ／ｍＬ,线性范围为１．５～３０００ｎｇ／ｍＬ;测定ＴＭＶ烟草病叶澄清液的最高稀释比为１∶１００００。检测灵敏度高于酶联免疫吸附显色光度法（ＥＬＩＳＡ）     

Fabrication of Active Horseradish Peroxidase Micropatterns with a High Resolution by Scanning Electrochemical Microscopy

We used a new reactive species OH^? to fabricate active horseradish peroxidase (HRP) micropatterns with a high resolution by scanning electrochemical microscopy (SECM) coupled with a carbon fiber disk electrode as the SECM tip. In this method, except for active HRP micropatterns predesigned other regions on a HRP‐immobilized substrate were deactivated by OH^? generated at the tip held at ?1.7 V in 1.0 mol/L KCl containing 2.0×10^?3 mol/L benzoquinone (BQ) (pH 8.0). The feedback mode of SECM with a tip potential of ?0.2 V was used to characterize the active HRP micropatterns in 1.0 mol/L KCl containing 2.0×10^?3 mol/L BQ and 2.0×10^?3 mol/L H₂O₂.     

Monitoring H2O2 on the Surface of Single Cells with Liquid Crystal Elastomer Microspheres

Live‐imaging of signaling molecules released from living cells is a fundamental challenge in life sciences. Herein, we synthesized liquid crystal elastomer microspheres functionalized with horse‐radish peroxidase (LCEM‐HRP), which can be immobilized directly on the cell membrane to monitor real‐time release of H₂O₂ at the single‐cell level. LCEM‐HRP could report H₂O₂ through a concentric‐to‐radial (C‐R) transfiguration, which is due to the deprotonation of LCEM‐HRP and the break of inter or intra‐chain hydrogen bonding in LCEM‐HRP caused by HRP‐catalyzed reduction of H₂O₂. The level of transfiguration of LCEM‐HRP revealed the different amounts of H₂O₂ released from cells. The estimated detection sensitivity was ≈2.2×10^?7 μm for 10 min of detection time. The cell lines and cell–cell heterogeneity was explored from different configurations. LCEM‐HRP presents a new approach for in situ real‐time imaging of H₂O₂ release from living cells and can be the basis for seeking more advanced chemical probes for imaging of various signaling molecules in the cellular microenvironment.     

Electrocatalytic determination of hydroquinone with Mn+ modified gold-5-amino-2-mercaptobenzimidazole self-assembled monolayer electrodes

Application of immobilized metal cations on the topside of gold-5-amino-2-mercaptobenzimidazole self-assembled monolayer (Au-5A2MBI-Mⁿ⁺ SAM, Mⁿ⁺:Cu²⁺ or Ag⁺) for electrocatalytic determination of hydroquinone (H₂Q) is described by voltammetric method. Several parameters were investigated to evaluate the performance of the sensors. Calibration curves for H₂Q concentrations were linear from 1.0 × 10^-5 to 4.0 × 10^-4 M (r = 0.998) for Au-5A2MBI, from 1.0 × 10^-5 to 6.0 × 10^-4 M (r = 0.998) for Au-5A2MBI-Cu²⁺, and from 2.0 × 10^-6 to 2.0 × 10^-5 M (r = 0.996) and 1.0 × 10^-4 to 1.0 × 10^-3 M (r = 0.991) for Au-5A2MBI-Ag⁺ SAM modified electrode. The respective detection limits were found as 6.5 × 10^-6, 4.6 × 10^-6 and 1.8 × 10^-7 M. Both Cu²⁺ and Ag⁺ ions were found to have a good electrocatalytic effect on the oxidation of H₂Q; however, Ag⁺ was a more effective catalyst and showed better sensitivity and lower detection limit than all other tested electrodes. Au-5A2MBI-Ag⁺ SAM electrode was used as a suitable sensor for determination of H₂Q in a radiolysis developing agent as real sample. The results obtained by using proposed sensor and that obtained by an ASTM reference method were in good agreement at the 95% confidence level.     

Mécanisme de réduction de l'ion molybdo-11 tungstique: (MoW11O40H2)6−

The reduction of the molybdotungstate ion: (MoW₁₁O₄₀H₂)^6? has been studied by polarographic, linear sweep voltammetric and spectrophotometric methods. Reduced products corresponding to 1, 2, 6, 10, 12 and 14 electrons per molecule of molybdotungstate have been prepared by electrolysis: some of their chemical and electrochemical properties (stability as a function of pH, disproportionation reactions) are described.     

A Sensitive Hydrogen Peroxide Sensor Based on Hemoglobin Immobilized on Gold Nanoparticles and 1,6-hexanedithiol Modified Gold Electrode

Hemoglobin (Hb) was successfully immobilized on a gold electrode modified with gold nanoparticles (AuNPs) via a molecule bridge 1,6-hexanedithiol (HDT). The AFM images suggested that the HDT/gold electrode could adsorb more AuNPs. UV-vis spectra indicated that Hb on AuNPs/HDT film retained its near-native secondary structures. The electrochemical behaviors of the sensor were characterized with cyclic voltammetric techniques. The resultant electrode displayed an excellent electrocatalytical response to the reduction of hydrogen peroxide (H₂O₂). The linear relationship existed between the catalytic current and the H₂O₂ concentration ranging from 5.0 × 10^?8 to 1.0 × 10^?6 mol · L^?1. The detection limit (S/N = 3) was 1.0 × 10^?8 mol · L^?1.